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Chicken Heat Shock Protein 90 Is a Component of the Putative Cellular Receptor Complex of Infectious Bursal Disease Virus▿

机译:鸡热激蛋白90是传染性法氏囊病病毒推定细胞受体复合物的组成部分▿

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摘要

Infectious bursal disease virus (IBDV) causes a highly contagious disease in young chicks and leads to significant economic losses in the poultry industry. The capsid protein VP2 of IBDV plays an important role in virus binding and cell recognition. VP2 forms a subviral particle (SVP) with immunogenicity similar to that of the IBDV capsid. In the present study, we first showed that SVP could inhibit IBDV infection to an IBDV-susceptible cell line, DF-1 cells, in a dose-dependent manner. Second, the localizations of the SVP on the surface of DF-1 cells were confirmed by fluorescence microscopy, and the specific binding of the SVP to DF-1 cells occurred in a dose-dependent manner. Furthermore, the attachment of SVP to DF-1 cells was inhibited by an SVP-induced neutralizing monoclonal antibody against IBDV but not by denatured-VP2-induced polyclonal antibodies. Third, the cellular factors in DF-1 cells involved in the attachment of SVP were purified by affinity chromatography using SVP bound on the immobilized Ni2+ ions. A dominant factor was identified as being chicken heat shock protein 90 (Hsp90) (cHsp90) by mass spectrometry. Results of biotinylation experiments and indirect fluorescence assays indicated that cHsp90 is located on the surface of DF-1 cells. Virus overlay protein binding assays and far-Western assays also concluded that cHsp90 interacts with IBDV and SVP, respectively. Finally, both Hsp90 and anti-Hsp90 can inhibit the infection of DF-1 cells by IBDV. Taken together, for the first time, our results suggest that cHsp90 is part of the putative cellular receptor complex essential for IBDV entry into DF-1 cells.
机译:传染性法氏囊病病毒(IBDV)在雏鸡中引起高度传染性疾病,并在家禽业造成重大经济损失。 IBDV的衣壳蛋白VP2在病毒结合和细胞识别中起重要作用。 VP2形成亚病毒颗粒(SVP),其免疫原性与IBDV衣壳相似。在本研究中,我们首先表明SVP可以剂量依赖性的方式抑制IBDV对IBDV易感细胞系DF-1细胞的感染。其次,通过荧光显微镜确认了SVP在DF-1细胞表面上的定位,并且SVP与DF-1细胞的特异性结合以剂量依赖性方式发生。此外,SVP诱导的针对IBDV的中和单克隆抗体抑制了SVP与DF-1细胞的附着,但变性的VP2诱导的多克隆抗体则没有抑制。第三,使用结合在固定的Ni 2+离子上的SVP通过亲和色谱法纯化参与SVP附着的DF-1细胞中的细胞因子。通过质谱鉴定,主要因素是鸡热激蛋白90(Hsp90)(cHsp90)。生物素化实验和间接荧光分析的结果表明cHsp90位于DF-1细胞的表面。病毒覆盖蛋白结合测定和远西方测定也得出结论,cHsp90分别与IBDV和SVP相互作用。最后,Hsp90和抗Hsp90均可抑制IBDV对DF-1细胞的感染。总而言之,我们的结果首次表明cHsp90是IBDV进入DF-1细胞必不可少的推定细胞受体复合物的一部分。

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